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Hindawi Publishing Corporation
Oxidative Medicine and Cellular Longevity
Volume 2013, Article ID 161986, 10 pages
http://dx.doi.org/10.1155/2013/161986
Research Article
Ammonium-Dependent Shortening of CLS in Yeast Cells
Starved for Essential Amino Acids Is Determined by the Specific
Amino Acid Deprived, through Different Signaling Pathways
Júlia Santos,1,2 Cecília Leão,1,2 and Maria João Sousa3
1
Life and Health Sciences Research Institute (ICVS), School of Health Sciences, University of Minho, 4710-057 Braga, Portugal
ICVS/3B’s-PT Government Associate Laboratory, Braga/Guimarães, Portugal
3
Molecular and Environmental Biology Centre (CBMA), Department of Biology, University of Minho, 4710-057 Braga, Portugal
2
Correspondence should be addressed to Maria João Sousa; [email protected]
Received 16 May 2013; Revised 9 July 2013; Accepted 16 July 2013
Academic Editor: Sergio Giannattasio
Copyright © 2013 Júlia Santos et al. This is an open access article distributed under the Creative Commons Attribution License,
which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
Ammonium (NH4 + ) leads to chronological life span (CLS) shortening in Saccharomyces cerevisiae BY4742 cells, particularly evident
in cells starved for auxotrophy-complementing amino acids (leucine, lysine, and histidine) simultaneously. Here, we report that the
effect of NH4 + on aging yeast depends on the specific amino acid they are deprived of. Compared with no amino acid starvation,
starvation for leucine alone or in combination with histidine resulted in the most pronounced NH4 + -induced CLS shortening,
whereas starvation for lysine, alone or in combination with histidine resulted in the least sensitivity to NH4 + . We also show that
NH4 + -induced CLS shortening is mainly mediated by Tor1p in cells starved for leucine or histidine but by Ras2p in cells starved
for lysine, and in nonstarved cells. Sch9p protected cells from the effect of NH4 + under all conditions tested (starved or nonstarved
cells), which was associated with Sch9p-dependent Hog1p phosphorylation. Our data show that NH4 + toxicity can be modulated
through manipulation of the specific essential amino acid supplied to cells and of the conserved Ras2p, Tor1p, and Sch9p regulators,
thus providing new clues to the development of environmental interventions for CLS extension and to the identification of new
therapeutic targets for diseases associated with hyperammonemia.
1. Introduction
In all living organisms, cell survival is mediated by metabolic
regulation in response to environmental conditions. This
regulation is conserved from yeasts to mammals and is mediated by complex nutrient signaling pathways that control
the necessary metabolic changes that take place when environmental conditions change [1]. In yeast, when nutrients
are depleted, cells undergo a growth arrest phase characterized by downregulation of growth signaling pathways and
upregulation of several processes, such as accumulation of
carbohydrates, autophagy, and stress resistance [2, 3]. The
length of time these nondividing yeast cells remain viable
for is defined as the chronological life span (CLS) of the
population [4]. The composition of the culture medium can
modulate CLS, and therefore, culturing cells in different
media leads to differences in CLS [5]. Manipulation of several
single components of the culture medium is known to extend
CLS, such as reducing glucose concentration (known as
caloric restriction-CR) or manipulating the supply of amino
acids [5–9]. Several studies in the literature report different
effects of amino acids on life span regulation, depending on
which amino acid is deprived [6–10]. In this context, it is
known that starvation for nonessential amino acids (strains
without auxotrophies) used as preferred nitrogen sources
can extend CLS [11–13], while starvation for auxotrophycomplementing amino acids (essential amino acids) reduces
CLS [7, 10]. However, not all essential amino acids contribute
equally to the effects on CLS. In fact, it has been described
that leucine plays a more important role in CLS extension
in auxotrophic strains [6, 10] and that extra supplementation
of leucine promotes CLS extension in standard 2% glucose
medium [6]. Recently, it has also been shown that leucine
influences autophagy and extension of CLS during CR [14].
2
The target of rapamycin complex 1 (TORC1) controls cell
growth in response to the availability of nutrients, including
amino acids [15, 16]. The TOR pathway responds to nitrogen
by regulating processes such as the transcription of genes
involved in nitrogen metabolism: nitrogen catabolite repression (NCR) sensitive genes, amino acid biosynthesis genes
(general amino acid control pathway-GAAC), retrograde
response genes (RTG-Pathway), and genes involved in the
stability of amino acid permeases and autophagy [17, 18]. In
mammalian cells, amino acids, predominantly leucine, regulate mTOR by controlling the ability of the positive regulator
Rheb-GTP to activate mTORC1. The fundamental role of
leucine in TORC1 regulation has been demonstrated through
the observation that withdrawal of leucine alone is almost
as effective in downregulating TORC1 as withdrawal of all
amino acids combined [19]. In yeast, the EGO complex is an
upstream regulator of TORC1, thought to be responsible for
amino acid signaling to TORC1. During leucine starvation,
TORC1 activation by this complex is disrupted, which results
in a reduction in Sch9p phosphorylation and slow growth
[20, 21].
The protein kinase A (PKA) pathway is involved in the
regulation of metabolism, stress response, and proliferation,
responding to the presence of a rapidly fermentable sugar and
other essential nutrients sustaining growth, such as amino
acids and phosphate [16, 22]. Readdition of nitrogen (amino
acids or ammonium) to cells starved for nitrogen activates
the PKA pathway through plasma membrane sensors known
as transceptors. Sch9p is a protein kinase that shares many
targets with PKA and TORC1, and different interactions
between these pathways, either cooperating or antagonizing
their effects, have been described [23]. It was shown that
Sch9p mediates PKA activation in the fermentable growth
medium induced (FGM) pathway, in response to amino acid
and ammonium, but not in phosphate-induced activation
[24].
We have previously shown that decreasing the ammonium (NH4 + ) concentration in the culture medium extends
the CLS of Saccharomyces cerevisiae BY4742 cells [25]. NH4 +
reduced the CLS of cells cultured to stationary phase under
both standard amino acid supplementation and amino acid
restriction conditions in a concentration-dependent manner,
and a significant increase in cell survival was observed
when the starting NH4 + concentration in the medium was
decreased. We also showed that when stationary phase cells
were transferred to water, the CLS was also significantly
shortened by addition of NH4 + , indicating that NH4 + alone
could induce the loss of cell viability observed in culture
media. The negative effects of NH4 + were particularly evident in cells cultured or incubated under restriction of
auxotrophy-complementing amino acid markers (leucine,
lysine, and histidine). These negative effects of NH4 + do
not appear to require its metabolization. The PKA and TOR
pathways were involved in NH4 + -induced CLS shortening,
but deleting SCH9 did not revert the decrease in cell viability
despite abolishing PKA activation in response to NH4 + ,
suggesting Sch9p plays an independent role in cell survival
[25].
Oxidative Medicine and Cellular Longevity
Here, we show that NH4 + toxicity during yeast aging
in water depends on the specific starved auxotrophy-complementing amino acid. Sch9p, contrary to Tor1p and Ras2p,
mediates cell survival in response to NH4 + in all starvation conditions through the phosphorylation of Hog1p. Our
results provide new insights in the modulation of CLS by
NH4 + , linking NH4 + toxicity to amino acid limitation. This
scenario of enhanced NH4 + toxicity in amino acid starvation
conditions is present in hyperammonemic patients, who are
often on dietary protein restriction [26]. The use of a simpler
model like yeast can help elucidate the underlying mechanism involved in the modulation of conserved signaling
pathways, in response to NH4 + .
2. Materials and Methods
2.1. Strains and Growth Conditions. Saccharomyces cerevisiae strain BY4742 (MATa his3Δ1 leu2Δ0 lys2Δ0 ura3Δ0)
(EUROSCARF, Frankfurt, Germany) and the respective
knockouts in HOG1, RAS2, SCH9, and TOR1 genes were used.
For experiments with nonstarved and amino-acid-starved
cells, the strains were first cultured at 26∘ C, 150 rpm, in
defined minimal medium (SC medium) containing 0.17%
yeast nitrogen base without amino acids and without
ammonium sulphate (Difco, BD), supplemented with 0.5%
(NH4 )2 SO4 , with appropriate amino acids and nucleotide
base (50 mg/L histidine, 50 mg/L lysine, 300 mg/L leucine,
and 100 mg/L uracil) and 2% D-glucose, to exponential
phase (OD600 = 1.0–1.5). These cells were harvested and
resuspended in (A) SC medium containing 4% glucose (nonstarved cells) or in (B) SC medium containing 4% glucose
and lacking (1) amino acids (aa-starved cells); (2) leucine
(Leu-starved cells); (3) histidine (His-starved cells); (4) lysine
(Lys-starved cells); (5) histidine and lysine (His-Lys-starved
cells); (6) leucine and lysine (Leu-Lys-starved cells), and
(7) leucine and histidine (Leu-His-starved cells). After 24
hours, cells were collected by centrifugation, washed three
times with water, and resuspended at a cell density of about
3.8 × 107 cells/mL in water (pH 7.0), or water with (NH4 )2 SO4
(0.5%, pH 7.0). Viability of 24-hour-starved cultures was
considered to be 100% of survival, and this was considered
day 0 of the experiment. pH 7.0 was maintained throughout
the experiment in cultures with adjusted pH. Cell viability of
culture aliquots was assessed by CFU at day 0 (100% viability)
and in subsequent days, as indicated. For CFU determination,
diluted samples were incubated for 2 days at 30∘ C on YEPD
agar plates.
2.2. Trehalase Activity. Trehalase activity was determined
according to [27]. Briefly, crude enzyme extracts were
obtained by resuspending the cell pellet in ice-cold 50 mM
MES/KOH buffer (pH 7.0) containing 50 𝜇M CaCl2 and
adding a roughly equal volume of 0.5 mm diameter glass
beads, followed by vigorous mixing during 1 minute intervals
interspersed with periods of cooling on ice. The extracts
were then dialyzed overnight at 4∘ C in a dialysis cellulose
membrane (Cellu Sep H1, Orange). The dialyzed extract
was then used to assess trehalase activity by measuring the
released glucose using a glucose oxidase assay (GOD, Roche).
Oxidative Medicine and Cellular Longevity
Protein concentration was determined using the Bradford
assay (Bio-Rad, Germany) according to the manufacturer’s
instructions.
2.3. Western Blot Analysis. Western blot analysis was performed according to [28]. Briefly, protein lysates were separated on 12.5% SDS-PAGE gels and transferred to polyvinylidene fluoride membranes (Hybond-P; Amersham). The
membranes were blocked with 5% bovine serum albumin
(BSA) in Tris-buffered saline (TBS, 50 mM Tris, 150 mM
NaCl, and pH 7.6) containing 0.05% Tween 20 for 1 h at room
temperature. Membranes were then incubated overnight at
4∘ C with primary antibodies directed against Hog1p (rabbit
anti-Hog1p MAPK; Santa Cruz Biotechnology, Inc., USA) at a
1 : 1000 dilution or rabbit anti-phospho-p38 MAPK (Cell Signaling Technology, Beverly, MA, USA) at a 1 : 50000 dilution
and against Pgk1p (mouse monoclonal anti-PGK1; Molecular
Probes) at a 1 : 5000 dilution. This was followed by a onehour incubation at room temperature with secondary antibody Peroxidase-AffiniPure Goat AntiRabbit IgG (1 : 10000;
Jackson ImmunoResearch) or Peroxidase-AffiniPure Goat
AntiMouse IgG (1 : 10000; Jackson ImmunoResearch).
3. Results and Discussion
3.1. 𝑁𝐻4 + -Induced Cell Death during Yeast Aging in Water
Depends on the Specific Auxotrophy-Complementing Amino
Acid Deprived from the Starvation Medium. In Saccharomyces cerevisiae BY4742, NH4 + leads to chronological life
span (CLS) shortening, particularly relevant in cells starved
for the auxotrophy-complementing amino acids simultaneously. The effect of NH4 + has been observed both in
cells aged in spent culture medium limited for the essential
amino acids and in cells aged in water after a 24-hour
incubation in amino-acid-deprived medium [25]. We now
sought to evaluate how the absence of specific auxotrophycomplementing amino acids affects NH4 + toxicity during
yeast CLS. For this purpose, cells were first grown to
exponential phase in SC medium and then starved for each
of the three essential amino acids of the BY4742 strain
(leucine, lysine, and histidine) alone or in combinations
of two, as well as in their absence (aa-starved cells). As
a control, we used the same medium, but without amino
acid deprivation, therefore adding the three auxotrophycomplementing amino acids (nonstarved cells). Cells were
then transferred to water with and without NH4 + , and cell
viability was evaluated over time. The protocol followed is
systematized in Figure S1 in Supplementary material available
online at http://dx.doi.org/10.1155/2013/161986.
The results presented in Figure 1(a) revealed that aa-,
lysine- (Lys-), or nonstarved cells displayed a longer CLS
in water without NH4 + than leucine- (Leu-) or histidine(His-) starved cells. Furthermore, absence of any of the three
amino acids in the medium, individually or at the same
time, decreased CLS upon transfer of cells to water with
NH4 + , in comparison with the CLS of cells incubaed without
amino acid restriction, though this effect was much less
accentuated when only lysine was removed (Figure 1(b)). Two
of the amino acids were then removed at the same time in
3
different combinations (Figures 1(c) and 1(d)). Simultaneous
absence of lysine and histidine (Lys-His-starved cells) had the
least effect on NH4 + -induced CLS shortening (Figure 1(d)),
whereas NH4 + was most toxic to cells starved both for
leucine and histidine (Leu-His starved cells). Comparing
these results with those from Figure 1(b) (removal of one
amino acid at a time from the medium), it can be observed
that survival of Leu- or His-starved cells in water with
NH4 + was much lower than that of cells that were also
starved for lysine (Leu-Lys- or His-Lys-starved cells). On
the other hand, the opposite effect was observed if Lysor His-starved cells were simultaneously starved for leucine
(Lys-Leu- or His-Leu-starved cells), where NH4 + -induced
CLS shortening was more severe. Additionally, histidine
starvation in combination with one of the other two amino
acids does not appear to have a major role in regulating CLS
in response to NH4 + , since the cell death profiles under those
conditions were similar to those exhibited by Lys- or Leustarved cells.
Taken together, the results suggest that from the three
auxotrophy-complementing amino acids tested, starvation
for leucine alone or in combination with histidine resulted
in the most severe effects on NH4 + -induced CLS shortening,
while starvation for lysine, alone or in combination with
histidine, resulted in the less sensitive NH4 + phenotype.
3.2. Ras2p, Tor1p, and Sch9p Differently Mediate 𝑁𝐻4 + Induced Cell Death during Yeast Aging in Water. The toxic
effects of NH4 + in aa-starved BY4742 cells are the result of
activation of the PKA and TOR pathways and are negatively
regulated by Sch9p [25]. In addition, the results shown in the
previous section demonstrated that ammonium affects CLS
shortening depending on the specific essential amino acid
deprived from the medium. We therefore sought to elucidate
the role of Ras2/PKA, Tor1p, and Sch9p signaling pathways
in CLS shortening induced by NH4 + under the different
starvation conditions. For this, we first tested the effect of
starving 𝑡𝑜𝑟1Δ, 𝑟𝑎𝑠2Δ, and 𝑠𝑐ℎ9Δ cells for each of the three
auxotrophy-complementing amino acids individually. As a
control, we used the same medium in the absence or presence
of all three essential amino acids. Similarly to what we
described above, cells were first grown to exponential phase
in SC medium, then incubated in the different starvation
media, and next transferred to water with or without NH4 +
(For schematic representation of the protocol please see
Figure S1).
The 𝑡𝑜𝑟1Δ strain displayed a lower NH4 + -induced cell
death than the wild-type strain in all starvation conditions
tested (Figures 1(b) and 2(b)). Furthermore, Lys-starved cells
displayed almost the same loss of cell viability as nonstarved
cells in the presence of NH4 + , showing that starvation for this
amino acid does not induce sensitivity to NH4 + in the absence
of TOR1. For nonstarved cells, there was no difference in the
effect of NH4 + between wild-type and 𝑡𝑜𝑟1Δ strains. On the
other hand, deletion of TOR1 also rescued the CLS of Hisstarved cells in water without NH4 + (Figures 1(a) and 2(a)).
In the 𝑟𝑎𝑠2Δ strain, the loss of cell viability induced
by NH4 + in nonstarved cells or Lys-starved cells was
significantly reduced when compared with the wild-type
Oxidative Medicine and Cellular Longevity
120
120
100
100
80
80
CFU counts (%)
CFU counts (%)
4
60
60
40
40
20
20
0
0
0
1
2
3
4
Time (days)
5
0
6
1
2
4
5
6
5
6
Time (days)
Non-starv. H2 O + NH4 +
aa-starv. H2 O + NH4 +
Leu-starv. H2 O + NH4 +
His-starv. H2 O + NH4 +
Lys-starv. H2 O + NH4 +
Non-starv. H2 O
aa-starv. H2 O
Leu-starv. H2 O
His-starv. H2 O
Lys-starv. H2 O
(a)
(b)
120
120
100
100
80
80
CFU counts (%)
CFU counts (%)
3
60
60
40
40
20
20
0
0
0
1
2
3
4
Time (days)
Non-starv. H2 O
aa-starv. H2 O
His-Lys-starv. H2 O
Leu-Lys-starv. H2O
Leu-His-starv. H2O
(c)
5
6
7
0
1
2
3
4
Time (days)
Non-starv. H2 O + NH4 +
aa-starv. H2 O + NH4 +
His-Lys-starv. H2 O + NH4 +
Leu-Lys-starv. H2 O + NH4 +
Leu-His-starv. H 2 O + NH4 +
(d)
Figure 1: Ammonium-induced cell death during yeast aging in water is dependent on the specific auxotrophy-complementing amino acid
deprived from the starvation medium. Survival of wild-type S. cerevisiae (BY4742) cells, nonstarved or starved for leucine, histidine, or lysine,
in different combinations upon ((a) and (c)) transfer to water (open symbol) or ((b) and (d)) water with (NH4 )2 SO4 , 0.5% (dark symbol). In
all the cultures, starting cell density was about 3.8 × 107 cells/mL, and the initial pH was adjusted to 7.0. Values are means ± SEM (𝑛 = 3).
(b) ∗∗ 𝑃 < 0.01 (aa-starved H2 O + NH4 + versus Lys-starved H2 O + NH4 + ), ∗∗ 𝑃 < 0.01 (aa-starved H2 O + NH4 + versus Leu-starved H2 O
+ NH4 + ), and ∗∗∗ 𝑃 < 0.001 (nonstarved H2 O + NH4 + versus Lys-starved H2 O + NH4 + ); (d) ∗ 𝑃 < 0.01 (nonstarved H2 O + NH4 + versus
His-Lys-starved H2 O + NH4 + ), ∗∗ 𝑃 < 0.01 (aa-starved H2 O + NH4 + versus Leu-His-starved H2 O + NH4 + ), and ∗∗∗ 𝑃 < 0.001 (aa-starved
H2 O + NH4 + versus His-Lys-starved H2 O + NH4 + ). Statistical analysis was performed by two-way ANOVA. All time points have error bars;
however, for time points with reduced standard error, they are not visible.
Oxidative Medicine and Cellular Longevity
5
tor1Δ
120
100
CFU counts (%)
100
CFU counts (%)
tor1Δ
120
80
60
40
80
60
40
20
20
0
0
0
1
2
3
4
Time (days)
5
6
0
1
2
(a)
100
CFU counts (%)
CFU counts (%)
80
60
40
80
60
40
20
20
0
0
1
2
3
4
Time (days)
5
6
0
1
2
(c)
3
4
Time (days)
5
6
5
6
(d)
sch9Δ
120
sch9Δ
120
100
100
CFU counts (%)
CFU counts (%)
6
ras2Δ
120
100
0
5
(b)
ras2Δ
120
3
4
Time (days)
80
60
40
20
80
60
40
20
0
0
1
2
3
4
Time (days)
Non-starv. H2 O
aa-starv. H2 O
Leu-starv. H2 O
His-starv. H2 O
Lys-starv. H2 O
(e)
5
6
0
0
1
2
3
4
Time (days)
Non-starv. H2 O + NH4 +
aa-starv. H2 O + NH4 +
Leu-starv. H2 O + NH4 +
His-starv. H2 O + NH4 +
Lys-starv. H2 O + NH4 +
(f)
Figure 2: Tor1p regulates ammonium CLS shortening in response to amino acid starvation. Survival of ((a) and (b)) tor1Δ, ((c) and (d))
ras2Δ, and ((e) and (f)) sch9Δ cells, nonstarved or starved for leucine, histidine, or lysine, individually or all at the same time, upon transfer
to water (open symbol) or water with (NH4 )2 SO4 , 0.5% (dark symbols). In all the cultures, starting cell density was about 3.8 × 107 cells/mL,
and the initial pH was adjusted to 7.0. Values are means ± SEM (𝑛 = 3). All time points have error bars; however, for time points with reduced
standard error, they are not visible.
6
strain. In contrast, deletion of RAS2 had only a slight effect
on the sensitivity of His- or Leu-starved cells to NH4 + , as well
as of cells starved for all three amino acids (aa-starved cells).
Furthermore, for the last two starvation conditions, deletion
of RAS2 induced a strong shortening of CLS in water without
NH4 + , indicating that Ras2p is important to ensure longevity
under these conditions (Figures 1(a) and 2(c)).
Absence of Sch9p reduced survival after cells were transferred to water with or without NH4 + for all conditions tested
(starved or nonstarved). Data from Figures 2(e) and 2(f) show
that Leu- or His-starved cells of the 𝑠𝑐ℎ9Δ strain behaved as
aa-starved cells when transferred to water with or without
NH4 + . In non- or Lys-starved cells, the loss of cell viability
in water, with or without NH4 + , was much less pronounced
than in the other starvation conditions, as observed for wildtype cells.
3.3. Ras2p, Tor1p, and Sch9p Mediate PKA Activation in
Response to 𝑁𝐻4 + during Yeast Aging in Water. To further
evaluate the role of PKA in NH4 + -induced CLS shortening
and the potential effects of Tor1p, Ras2p, and Sch9p as PKA
upstream regulators, we assessed PKA activation in BY4742
(wild-type), 𝑡𝑜𝑟1Δ, 𝑟𝑎𝑠2Δ, and 𝑠𝑐ℎ9Δ strains starved for
each of the three essential amino acids, individually or in
combination. Trehalase is a target of PKA regulation, and its
activity has been extensively used to monitor PKA activation
[22, 29]. In order to evaluate PKA activation, we therefore
measured trehalase activity in cells grown and incubated
as described above in material and methods section. (For
schematic representation of the protocol please see Figure
S1). We observed that in wild-type cells, leucine starvation
resulted in the highest trehalase activity after 2 h of incubation
with NH4 + , whereas its presence alone led to the lowest
trehalase activity. In contrast, and under the same conditions,
starvation for lysine or histidine alone gave rise to the
lowest trehalase activity, whereas their presence alone led
to the highest trehalase activity (Figure 3(a)). The results
also showed that in the presence of NH4 + , aa-starved cells
exhibited a PKA activation pattern similar to nonstarved
cells, with values that are between those obtained for Leuand His- or Lys-starved cells. This suggests that in aastarved cells, the higher contribution expected from PKA
activation due to the absence of leucine is probably balanced
by the decrease of PKA activity induced by the absence of
histidine and lysine. PKA activation by NH4 + was decreased
in 𝑡𝑜𝑟1Δ, 𝑟𝑎𝑠2Δ, and 𝑠𝑐ℎ9Δ mutants in comparison with
the wild-type strain, both for nonstarved cells and under
all amino acid starvation conditions (Figures 3(b), 3(c), and
3(d)). The observed reduction in PKA activation correlates
with the decrease in NH4 + -induced CLS shortening in the
𝑡𝑜𝑟1Δ strain under all the conditions tested. In addition,
the decrease in PKA activation induced by NH4 + in the
ras2Δ strain was accompanied by an increase in cell survival
for non- or lysine-starved cells, but not for cells under the
remaining starvation conditions (Leu-, His-, or aa-starved
cells). Conversely, for nonstarved cells and for cells starved
in the presence of leucine (His-starved and Lys-starved cells)
before transfer to water (T0), there was a significant increase
in PKA activation in the 𝑟𝑎𝑠2Δ strain, indicating that Ras2p
Oxidative Medicine and Cellular Longevity
seems to downregulate PKA activity in the presence of
leucine. On the other hand, the decrease in PKA activation
induced by NH4 + in the sch9Δ strain was not associated
with an extended CLS in water with NH4 + in nonstarved
cells or under any of the starvation conditions tested, which
is in accordance with previous results described for aastarved cells [25]. Together, the results suggest that NH4 +
induces PKA activation through Tor1p, Ras2p, and Sch9p.
However, absence of Ras2p, although able to decrease PKA
activation, did not revert NH4 + -induced CLS shortening
in Leu-, His-, and aa-starved cells, indicating that in the
absence of this protein, other pathways, independent of PKA
and possibly mediated by Tor1p, are still activated and can
induce cell death. Furthermore, Ras2p, at least under some
conditions, appears to also activate other pathways relevant
to cell survival, since its absence leads to a shorter CLS in
water. A prosurvival role was also observed for Sch9p under
all conditions, either in the absence or presence of NH4 + .
3.4. Sch9p Protects Cells from 𝑁𝐻4 + -Induced Cell Death
through Hog1p Activation. Hog1p is a kinase that regulates
and is regulated by Sch9p and mediates stress response
independently of the PKA and TOR pathways [30]. It was
previously shown that Hog1p is involved in the resistance of
aa-starved cells to the toxic effects of NH4 + during CLS in
water [25]. In order to access if the protective role of Sch9p
in response to NH4 + under the different amino acid starvation conditions described in the previous sections could be
mediated through a Sch9p-dependent Hog1p activation, we
examined Hog1p phosphorylation during CLS in water with
and without NH4 + in BY4742 (wild-type) and 𝑠𝑐ℎ9Δ cells. As
shown in Figure 4, Hog1p phosphorylation in wild-type cells
increased in the presence of NH4 + in all starvation conditions
tested (aa-, Leu-, His-, and Lys-starved cells), being higher in
His- and Lys-starved cells. Deletion of SCH9 almost abolished
Hog1p phosphorylation in aa-, Leu-, and His-starved cells,
whereas some residual phosphorylation was still detected in
Lys-starved cells. The lower Hop1p phosphorylation observed
for cells starved for aa- and Leu-starved cells is in agreement
with previous results, showing that the presence of leucine
is required for Sch9p phosphorylation via TORC1 [21]. Also,
Hog1p phosphorylation in Lys-starved 𝑠𝑐ℎ9Δ cells is in agreement with the activation of pathways other than the PKA in
the absence of Ras2p, suggested by the rescue of the loss of
viability found for Lys-starved 𝑟𝑎𝑠2Δ cells (Figure 2(d)).
Taken together, results show that Sch9p is involved in
Hog1p activation in response to NH4 + under all starvation
conditions, indicating that the increased resistance afforded
by Sch9p could, actually, be mediated through Hog1p activation.
4. Conclusions
It has been previously shown that the CLS of stationary phase
cells of Saccharomyces cerevisiae BY4742 transferred to water
was significantly shortened by the addition of NH4 + and
that the negative effects of NH4 + were particularly evident
for cells under restriction of auxotrophy-complementing
amino acid markers (leucine, lysine, and histidine) [25]. The
Oxidative Medicine and Cellular Longevity
7
tor1Δ
∗
25
20
15
10
25
20
15
10
5
T0 h
T2 h H2 O
T2 h H2 O + NH4 +
T0 h
T2 h H2 O
T2 h H2 O + NH4 +
(b)
(a)
40
∗∗∗
Trehalase sp. act.
(nmol min−1 (mg protein)−1 )
60
40
30
20
10
35
30
25
20
15
10
5
∗
Lys-starv.
His-starv.
Leu-starv.
aa-starv.
Non-starv.
aa-starv.
0
0
Non-starv.
Trehalase sp. act.
(nmol min−1 (mg protein)−1 )
70
sch9Δ
Leu-starv.
ras2Δ
80
Lys-starv.
Non-starv.
His-Lys-starv.
30
0
Leu-His-starv.
His-starv.
Leu-starv.
aa-starv.
Non-starv.
0
Leu-Lys-starv.
5
35
His-starv.
∗∗
T0 h
T2 h H2 O
T2 h H2 O + NH4 +
T0 h
T2 h H2 O
T2 h H2 O + NH4 +
(c)
(d)
Lys-starv.
∗∗
Leu-starv.
30
∗∗
His-starv.
∗
aa-starv.
35
Trehalase sp. act.
(nmol min−1 (mg protein)−1 )
40
Lys-starv.
Trehalase sp. act.
(nmol min −1 (mg protein)−1 )
40
Figure 3: Ammonium induction of PKA activity depends on Tor1p, Ras2p and Sch9p regulation. Trehalase activity of cells nonstarved or
starved for leucine, histidine, or lysine, individually or in different combinations, of (a) wild-type S. cerevisiae (BY4742) and of mutant deleted
strains (b) tor1Δ, (c) ras2Δ, and (d) sch9Δ; before being, transferred to water (T0h) and after 2 hours in water (T2h H2 O) or water with
(NH4 )2 SO4 , 0.5% (T2h H2 O + NH4 + ). In all the cultures, starting cell density was about 3.8 × 107 cells/mL, and the initial pH was adjusted
to 7.0. Values are means ± SEM (𝑛 = 3–4). (a) ∗ 𝑃 < 0.05 (aa-starved T0h versus aa-starved T2h H2 O + NH4 + ), ∗∗ 𝑃 < 0.01 (Leu-starved
T0h versus Leu-starved T2h H2 O + NH4 + ), ∗∗ 𝑃 < 0.01 (Leu-starved T2h H2 O + NH4 + versus His-starved T2h H2 O + NH4 + ), ∗∗ 𝑃 < 0.01
(Leu-starved T2h H2 O + NH4 + versus Lys-starved T2h H2 O + NH4 + ), ∗ 𝑃 < 0.05 (Leu-starved T2h H2 O + NH4 + versus His-Lys-starved T2h
H2 O + NH4 + ); (c) ∗∗∗ 𝑃 < 0.001 (nonstarved T0h versus nonstarved H2 O + NH4 + ); (d) ∗ 𝑃 < 0.05 (aa-starved T0h versus aa-starved T2h
H2 O + NH4 + ). Statistical analysis was performed by two-way and one-way ANOVA.
results presented herewith demonstrate that NH4 + -induced
cell death during aging in water depends on the specific
auxotrophy-complementing amino acid deprived from the
starvation medium. While Lys-starved cells were only slightly
more sensitive to NH4 + -induced CLS shortening than nonstarved cells, Leu- and His-starved cells displayed a much
stronger sensitivity to NH4 + during CLS, which was comparable to that previously described for cells simultaneously
starved for all three essential amino acids (aa-starved cells).
When we compare cells starved for one amino acid at a time
with nonstarved cells, absence of any of the three auxotrophycomplementing amino acids from the medium has a detrimental effect leading to a faster loss of cell survival in response
to ammonium. However, when cells are starved for at least
one amino acid, the presence of lysine in the medium is
detrimental, histidine does not seem to have an effect, and
8
Oxidative Medicine and Cellular Longevity
aa-starvation
Leu-starvation
sch9Δ
WT
C
WT
sch9Δ
+
+
+
+
NaCl T0 H2 O NH4 T0 H2 O NH4 T0 H2 O NH4 T0 H2 O NH4
Pi-Hog1p
Hog1p
Pgk1p
(a)
His-starvation
WT
C
Lys-starvation
sch9Δ
WT
sch9Δ
+
+
+
+
NaCl T0 H2 O NH4 T0 H2 O NH4 T0 H2 O NH4 T0 H2 O NH4
Pi-Hog1p
Hog1p
Pgk1p
(b)
Figure 4: Ammonium induces Sch9p-dependent Hog1p phosphorylation in starvation conditions. Westernblot analysis of Pi-Hog1p levels
present in S. cerevisiae (BY4742) wild-type (WT) and sch9Δ cells starved for (a) all three amino acids or leucine and (b) starved for histidine
or lysine, before (T0) and after 20 minutes upon transfer to water (H2 O) or water with (NH4 )2 SO4 , 0.5% (NH4 + ). In all the cultures, starting
cell density was about 3.8 × 107 cells/mL, and the initial pH was adjusted to 7.0. Control cells were grown on YPD medium (Control-C) and
incubated for 5 minutes in YPD medium supplemented with 1 M NaCl.
leucine has a protective effect on ammonium-induced CLS
shortening. The results regarding leucine are in accordance
with the literature since it has been described that leucine
plays a more important role in CLS extension in auxotrophic
strains [6, 10]. In a recent study, supplementation of extra
leucine to SC medium or transformation of auxotrophic
leucine strain into a prototrophic leucine strain resulted in
CLS extension. The importance of leucine was attributed
to the regulation of the branched side chain amino acids
synthesis that appears to be misregulated in a leu2Δ strain.
In agreement, supplemental levels of the branch side amino
acids isoleucine, threonine, and valine also extended CLS in
a leu2Δ strain [6]. The negative effect observed for lysine
in cell survival during ammonium-induced cell death can
possibly be due to the fact that autophagy is inhibited in
the presence of ammonium [25], and the lack of autophagy
might be responsible for this effect since lysine seems to act
in an autophagy-dependent manner on the regulation of CLS.
Autophagy-deficient strains showed no improvement in CLS
extension after regaining LYS prototrophy in contrast to wildtype autophagy competent cells that increased CLS extension
with LYS prototrophy [6].
Both Ras2p and Tor1p are involved in NH4 + -induced
CLS shortening in aa-starved cells [25]. We now further
established that Ras2p involvement on NH4 + -induced CLS
shortening was present under all conditions tested, and did
not depend on starvation. In turn, Tor1p function in the
decrease of CLS by NH4 + was relevant only under amino acid
starvation, being differently modulated by the specific amino
acid deprived from the medium. Starvation for leucine and
histidine, which induced a strong shortening of CLS in the
presence of NH4 + , had a high impact in the regulation of
Tor1p function, whereas starvation for lysine, which was associated with only a small NH4 + -induced CLS shortening, had
a considerably less significant impact on Tor1p regulation.
These results are in agreement with previous results showing
that leucine has an important impact in the regulation of
TORC1 [20, 21]. Our results suggest that the presence of NH4 +
in the medium (commonly present as the nitrogen source)
may be at least partly responsible for the reported decrease in
CLS in leucine-starved cells [6, 14].
PKA activation has been described to be associated
with the NH4 + -induced CLS shortening of aa-starved cells
in water [25]. From the results now obtained, and when
we compare values from nonstarved and starved wildtype cells, it appears that leucine starvation (alone or in
combination with starvation for another amino acid) is the
main factor responsible for PKA activation in response to
Oxidative Medicine and Cellular Longevity
NH4 + , correlating with its stronger effect on CLS shortening.
This activation is dependent on Ras2p, Tor1p, and Sch9p,
as deficiency in any of these proteins leads to its decrease.
However, since the decrease in PKA activation resulted in
distinct cell fate outcomes in the different mutants, the results
suggest that these proteins activate PKA by independent
pathways and/or also regulate other pathways that they do
not share and that have different impacts on NH4 + -induced
CLS shortening. Also, we cannot exclude the possibility that
the observed effects on trehalase activity may result from a
potential effect of Sch9p, Ras2p, or Tor1p on the activity of
other proteins also involved in trehalase regulation such as
Bmh1/2p or Dcs1p [29].
Opposite to our results, Sch9p has been described to
inhibit PKA activity when glucose is added to glycerol-grown
cells. However, these authors observed that the inhibition
was mediated through the regulation of Tpk2p localization
[31], an isoform that does not seem to have a relevant role
in response to ammonium under our conditions. In fact,
we have previously observed that Tpk1p is the main PKA
isoform involved in ammonium effects [25]. In addition to its
involvement in PKA activation, Sch9p also increases Hog1p
phosphorylation, extending CLS in water with or without
NH4 + .
In summary, herewith we show that the toxic effects
of NH4 + on CLS shortening are regulated by a starvationdependent and a starvation-independent component and are
mediated essentially by Tor1p in the first case and by Ras2p
in the second. We also provide evidence that when cells
are starved for amino acids, the presence of leucine can
ameliorate NH4 + -induced CLS shortening, while lysine has
the opposite effect, and the presence of histidine has no effect.
Together, our data add new knowledge on CLS regulation,
indicating that the modulation of nitrogen sources supplied
to cells can drastically modulate CLS and providing new
clues for the development of environmental interventions
for chronological life span extension. Additionally, and since
NH4 + -induced cell death is involved in different human
disorders that are accompanied by hyperammonemia [32],
our results, showing that NH4 + toxicity can be modulated by
amino acids through different pathways, may also afford new
insights into the understanding of the cell molecular bases
triggering cell death in such pathologies.
Authors’ Contribution
9
[2]
[3]
[4]
[5]
[6]
[7]
[8]
[9]
[10]
[11]
[12]
[13]
Maria João Sousa and Cecı́lia Leão contributed equally to this
work.
Acknowledgment
This work was supported by FCT, Portugal, Grant PTDC/
AGR-ALI/102608/2008.
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